利用嗜热热菌宿主载体系统表达嗜热古细菌堀氏焦球菌的基因

G. Takayama, T. Kosuge, S. Sunamura, I. Matsui, K. Ishikawa, A. Nakamura, T. Hoshino
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引用次数: 6

摘要

利用嗜热古细菌horikoshipyrococcus OT3中苏氨酸脱氢酶、α-甘露糖苷酶和谷氨酸脱氢酶的注释基因,检测嗜热真细菌Thermus thermophilus HB27的表达系统。使用先前描述的P215启动子,这三个基因成功表达,但其表达水平明显低于使用T7启动子的大肠杆菌表达系统。用P31或Pslp_promoter替换启动子区域,将表达提高到与大肠杆菌系统相当或超过的水平。值得注意的是,α-甘露糖苷酶活性可以通过P31和pslp_启动子清楚地检测到,而在大肠杆菌系统中无法检测到。此外,在这些酶的COOH-或nh2端有6次His-tag的融合,通过Western blotting可以在嗜热T.的粗提取物中检测到这些蛋白,这表明每种酶活性的增加实际上是酶生产的结果。这些结果表明嗜热T.嗜热菌的宿主-载体系统对嗜热T.嗜热菌基因的表达是有用的。
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Use of a Thermus thermophilus host-vector system for expression of genes from the hyperthermophilic archaeon Pyrococcus horikoshii
Genes annotated to threonine dehydrogenase, α-mannosidase, and glutamate dehydrogenase of the hyperthermophilic archaeon Pyrococcus horikoshii OT3 were used to test the expression system of the thermophilic eubacterium Thermus thermophilus HB27. Using the previously described P215 promoter, the three genes were successfully expressed, but at significantly lower levels than in the Escherichia coli expression system with the T7 promoter. Replacement of the promoter region with P31 or Pslp_promoter improved the expression to a level comparable to or exceeding that in the E. coli system. Notably, α-mannosidase activity was clearly detected with the P31 and Pslp_promoters, which could not be detected in the E. coli system. Moreover, with 6 x His-tag fusions of these enzymes at their COOH- or NH2-termini, these proteins could be detected in the crude extracts of T. thermophilus by Western blotting, indicating that the increment of each enzyme activity was actually the result of enzyme production. These results demonstrate that the host-vector system of T. thermophilus is useful for expression of genes from hyperthermophiles.
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